Eugenol as a potential adjuvant therapy for gingival squamous cell carcinoma

Adoption of plant-derived compounds for the management of oral cancer is encouraged by the scientific community due to emerging chemoresistance and conventional treatments adverse effects. Considering that very few studies investigated eugenol clinical relevance for gingival carcinoma, we ought to explore its selectivity and performance according to aggressiveness level. For this purpose, non-oncogenic human oral epithelial cells (GMSM-K) were used together with the Tongue (SCC-9) and Gingival (Ca9-22) squamous cell carcinoma lines to assess key tumorigenesis processes. Overall, eugenol inhibited cell proliferation and colony formation while inducing cytotoxicity in cancer cells as compared to normal counterparts. The recorded effect was greater in gingival carcinoma and appears to be mediated through apoptosis induction and promotion of p21/p27/cyclin D1 modulation and subsequent Ca9-22 cell cycle arrest at the G0/G1 phase, in a p53-independent manner. At these levels, distinct genetic profiles were uncovered for both cell lines by QPCR array. Moreover, it seems that our active component limited Ca9-22 and SCC-9 cell migration respectively through MMP1/3 downregulation and stimulation of inactive MMPs complex formation. Finally, Ca9-22 behaviour appears to be mainly modulated by the P38/STAT5/NFkB pathways. In summary, we can disclose that eugenol is cancer selective and that its mediated anti-cancer mechanisms vary according to the cell line with gingival squamous cell carcinoma being more sensitive to this phytotherapy agent.


MTT proliferation and viability assay
The cells were seeded in 24 well plates and incubated with the 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide MTT agent (Sigma-Aldrich, M-2128) diluted at 0.5 mg/ml for 3 h.The plates were then covered and kept in the incubator at 37 °C to allow reduction of the yellow tetrazolium salt to purple formazan crystals by metabolically active cells.The insoluble crystals were dissolved by using the isopropanol 0.4% HCl and the optic density was measured at 550 nm using the Bio-Rad xMark™ Microplate Absorbance Spectrophotometer.IC50 is defined as the half maximal inhibitory concentration required to inhibit a biological process by half.Three technical replicates and four biological replicates were carried out.

LDH cytotoxicity assay
The Lactate dehydrogenase LDH kit (Roche, 11644793001) was used according to the manufacturer's instructions to assess cytotoxicity levels.Dye and catalyst solutions were added to culture supernatants for 30 min.The formation of the red formazan product being directly proportional to the enzyme released ensured quantification of the extracellular LDH released upon damage to plasma membrane.Optic density was measured at 490 nm by the means of the Bio-Rad xMark™ Microplate Absorbance Spectrophotometer.Three technical replicates and four biological replicates were carried out.

Colony formation assay
The cells were grown for 14 days to allow colony formation in the presence or absence of different concentrations of eugenol then they were rinsed twice with PBS before being fixed with cold methanol for 10 min.1% Crystal violet (Sigma-Aldrich, 548-62-9) was added for another 10 min and the excess of the product was washed away using water.Colonies were photographed to show differences at this level.Four biological replicates were carried out.

Annexin V/propidium iodide apoptosis test
Following treatment with eugenol, dead cells populations were analyzed using the APC Annexin V apoptosis detection kit with PI (Biolegend, 640932).After 24 h of eugenol treatment, the apoptosis and necrosis markersannexin V (AnxV) and propidium iodide (PI)-were incubated with the cells for 20 min at room temperature.Analysis with the BD FACSCanto II flow cytometry system permitted events classification as viable (AnxV−/PI−), early apoptotic (AnxV+/PI−), late apoptotic (AnxV+/PI+) and necrotic cells (AnxV−/PI+).Three biological replicates were carried out.

QPCR arrays
RT 2 Profiler PCR arrays corresponding to human cell cycle (Qiagen, PAHS-020ZD-6) and apoptosis (Qiagen, PAHS-012ZD-6) served to unravel key determinants implicated in cancer progression.The acquired data was analyzed using the 2-ΔΔCT method to determine relative gene expression and the fold changes between nonexposed and eugenol-treated cells.A gene was considered upregulated or downregulated when the fold change exceeded twice the initial value.CT values were extracted and compiled into a table, which was subsequently uploaded to the web portal for data analysis, accessible at http:// www.qiagen.com/ geneg lobe.The values obtained were normalized based on an automated selection from a comprehensive set of reference genes.This indicative study corresponds to only one experiment.

Cell cycle distribution
Cells were treated with different concentrations of eugenol for 24 h then exposed to the action of trypsin.Harvested cells were washed, fixed in cold 70% ethanol for 1 h then exposed to the action of ribonucleases (Roche, 93137524) to ensure only the DNA is stained by propidium Iodide (Biolegend, 640932).The later was incubated with the cells for 20 min at room temperature.Analysis using the BD FACSCanto II flow cytometry system allowed classification according to the cell cycle phase.Three biological replicates were carried out.

Scratch assay
A simple scratch was created in cell monolayer and the capacity of the cells to migrate in the presence of different eugenol concentrations was studied.Images were taken with the Nikon ECLIPSE TS100 optical microscope at two time points: the beginning of the experiment then after 24 h.The microscope magnification was set at × 10.At the end point, cells were stained with crystal violet as previously described to obtain better quality photos under the microscope.Scratch diameter was measured using the Lumenera infinity analyze 6.5.5 software to quantify the scratch healing process.Three to four biological replicates were carried out.

Gelatin zymography
Polyacrylamide gels containing 1% gelatin (J.T.Baker, 424865) allowed to screen for MMP-2 and MMP-9 gelatinase enzymes in cell supernatants.Samples were prepared in a standard non reducing buffer and subjected to electrophoresis.SDS was removed from the gels by the action of the 2.5% triton X-100 washing solution.The later was replaced by the developing buffer so that gelatin digestion can occur overnight at 37 °C.Gels were then stained following 30 min exposure to Coomassie Brilliant Blue R-250 (Bio-Rad, 161-0436) and bands detection was warranted after incubation with the de-staining buffer consisting of 25% methanol 10% acetic acid.Three to four biological replicates were carried out.

Flow cytometry analysis of signaling pathways
As previously described by our team 25 , cells were washed then fixed in 1.5% paraformaldehyde for 20 min at room temperature.Cells were re-rinsed and permeabilized using a 90% methanol/PBS solution.This step was realized on ice for a total period of 20 min.An additional wash cycle was performed, and cells were labeled for 30 min using the following fluorescence conjugated primary antibodies: pSTAT1 (BD Biosciences, AB_1645373), pSTAT3 (BD Biosciences, AB_647232), pSTAT5 (BD Biosciences, AB_399858), pERK1/2 (BD Biosciences, AB_399857), phosphorylated p38 (BD Biosciences, AB_399856) and Phospho NF-κB p65 (Thermofisher, AB_2572751).Cells were washed for the last time and flow cytometry analysis using the BD Accuri C6 Plus flow cytometer allowed estimation of ERK1/2, NF-κB, STAT1, STAT3, STAT5 and P38 phosphorylation levels.The histogram subtraction technique was applied based on Overton subtraction and thus the overlay of the histograms of interest.The analysis was then realized by the FCS express De Novo software 42 .Three biological replicates were carried out.

Eugenol induces cytotoxicity and hinders cell proliferation as well as colony formation
Eugenol treatment counteracts Ca9-22 and SCC-9 proliferation in a dose dependent manner with gingival cell line being more sensitive to treatment.This is clearly showing following supplementation of high eugenol concentrations.IC50, also known as the half maximal inhibitory concentration, is recorded around 200 µM for Ca9-22 and 300 µM for SCC-9.Interestingly, our phytotherapy agent was unfolded as cancer selective (Fig. 1A).This is also showing at the level of the LDH assay where little cytotoxicity was linked to the GMSM-K normal cells as compared to the Ca9-22 and SCC-9 models (Fig. 1B).Moreover, crystal violet staining demonstrated complete abolition of colony formation at concentrations as low as 200 µM.In this respect, a repressive effect is detected at 100 µM for Ca9-22 (Fig. 1C).

Eugenol exhibits its effects on gingival carcinoma through cyclin D1 modulation and subsequent cell cycle arrest at the G0/G1 phase
Treatment with increasing concentrations of eugenol for 24 h favored Ca9-22 cell cycle arrest at the G0-G1 phase.In further detail, we can state that relative to the control condition, it is evident that the percentage of the cells blocked in the G0-G1 phase scored 28,9% increase when administering our phytotherapy agent at concentrations as little as 100 µM (Fig. 2A and B).The half maximal inhibitory concentration (IC50) was then  1).The modified factors corresponded to key G1 phase markers, S phase components, DNA repair agents and controllers of G1/S transition (Fig. 2E).On the other hand, it is worth noting that for the same outcome, which is eliminating half of the exposed oral cancer cells, eugenol follows a different path in tongue carcinoma cell line.More specifically, distinct profiles were uncovered for both cell lines by QPCR array and eugenol induced a blockade, most likely, post-G1 for SCC-9 (Supplementary Table 1).

Eugenol significantly induce Ca9-22 cells apoptosis
Following supplementation of eugenol, the percentage of dead cells populations mainly the Anx V+/PI+ late apoptotic cells was significantly increased in a dose dependent manner (Fig. 3A and B).More specifically, the percentage of apoptotic cells changed from 16.8 to 86.7% upon treatment with 400 µM of eugenol.Due to the action of our polyphenol, the protein expression levels of Noxa and pro-PARP1 were significantly decreased (Fig. 3C and Supplementary Fig. 3).Based on QPCR array data, it was revealed that a total of 31 apoptotic genes are modulated by the supplementation of eugenol.More specifically, 20 factors were shown to be upregulated.2).Importantly, discrepancies between oral carcinoma cell lines were once more detected and a different genetic profile was revealed for the SCC-9 cell line (Supplementary Table 2).

Eugenol limits Ca9-22 cell migration through MMP1/3 downregulation
Scratch assay data analysis demonstrated that eugenol limited Ca9-22 cells migration and thus healing in a dose dependent manner.Scratch closure is totally marked in the control, whereas following stimulation with 100 µM eugenol, an inhibition of Ca9-22 migration potential by 53% was recorded, in the absence of any significant impact on cytotoxicity as well as on cell proliferation (Fig. 4A and B).To understand the underlying mechanisms, we then focused on the members of several secreted protease groups including the MMP1 collagenase, the MMP2/9 gelatinases and the MMP3 stromelysin given the diversity of the substrate range 43 .As per the gelatin zymography and QPCR results, it appears that this effect is not mediated through MMP2 and MMP9 modulation (Fig. 4C and Supplementary Fig. 5) but rather associated to MMP1 and MMP3 elimination (Fig. 4D and  E).Even though eugenol exhibited the same impact on SCC-9 migration, the causal processes were shown to be different and inactive MMPs complex formation is detected.No effect at the level of MMP1, MMP2 and MMP9 expression was recorded.Only MMP3 upregulation was observed following treatment with 300 µM eugenol (IC 50 for SCC9) (Supplementary Fig. 4 and 5).

Eugenol effects are mediated by pSTAT5, pP38, pNF-kB modulation
Flow cytometry results showed that supplementation with 200 µM eugenol for 24 h stimulated the phosphorylation of STAT5 (Fig. 5A) and P38 (Fig. 5B).Phospho-NF-ĸB levels on the other hand were negatively regulated (Fig. 5C).A slight effect was detected at the level of pSTAT1 and pERK1/2 (data not shown).It seems that gingival and tongue carcinoma modulate distinct signaling molecules as no effect was shown on the phosphorylated forms of the aforementioned signaling molecules following incubation with 300 µM eugenol.Only a miniscule increase of STAT3 phosphorylation was discovered (data not shown).

Discussion
Despite current use in dental clinics for its antibacterial effect, eugenol implication as an alternative treatment option for cancer is beginning to gain ground in research.In fact, eugenol effectiveness towards various cancer models including melanoma, leukemia and skin tumors was previously validated 32   www.nature.com/scientificreports/ of eugenol dental compound against human oral squamous cell carcinoma cell lines HSC-2, HSC-4 and Ca9-22 and this is relative to normal cells and other anticancer drugs 44 , Surducan et al. were able to report inhibition of SCC-4 tongue carcinoma proliferation in a dose dependant manner.IC50 was registered around 750 µM and a high concentration, in the order of 500 µM, was required to induce apoptosis 38 .In another paper, eugenol decreased colony formation and around 900 µM was needed to eliminate half of the SCC-9 cells 37 .This was to be expected as tongue carcinoma is generally regarded as a more aggressive and a highly metastatic entity as opposed to other oral subsites 45 .For instance, cervical lymph node metastasis, greatly correlated with tongue tumors, is known to reduce survival chances half 6,8,46 .In the present study, we focused on eugenol effectiveness against a less aggressive form occurring in the gingival tissue.Our results showed that eugenol inhibited Ca9-22 oral cancer cells proliferation, and that the effect registered was more remarkable as compared to tongue carcinoma.Tumor specific IC50s were recorded around 200 µM for Ca9-22 and 300 µM for the SCC-9 cell line.Being selective to the Ca9-22 cancer cells, this paper is encouraging the potential use of eugenol for the specific management of gingival carcinoma and is aiming to decipher its mechanisms of action.
Given that eugenol was proven to be capable of inducing cytotoxicity and hindering cell proliferation and colony formation, it was imperative to test whether the observed outcomes were mediated by a direct impact on the progression of the cell cycle.Interestingly, we were able to confirm a blockade of Ca9-22 cells at the level of G0-G1 following supplementation of eugenol.Based on our QPCR array data, the tongue carcinoma cell line reacted in a different way.At this level, Saranya Varadarajan et al. showed that Cinnamomum verum J. Presl extract (bark) and its active constituents including eugenol demonstrated anticancer effects in vitro via apoptosis induction and S-phase arrest of the SCC-25 tongue carcinoma cell line 39 .Considering the novelty of the Table 2. Effect of eugenol on gene expression profile of apoptotic Ca9-22.QPCR array data corresponding to apoptotic genes expression profile.A total of 84 markers were analyzed following incubation with an intermediate concentration of eugenol estimated at 200 µM.The treatment duration was limited to 24 h.Unigene designator, Refseq identifier, symbol and description corresponding to all factors showing discrepancies relative to untreated control are summarized in Table 2.Only the genes displaying over two-fold variation were taken into consideration.This indicative study corresponds to only one experiment (n = 1).subject, it was important to focus on analyzing the determinants of Ca9-22 response to eugenol.Based on the western blot and QPCR array data, we were able to unravel key G1 phase markers, S phase components, DNA repair agents and controllers of G1/S transition implicated at this level.Primarily, we were able to show reduced expression of the cyclin dependent kinases (CDK) 4/6 and of their allosteric activator cyclin D1.Being a driver of G1/S transition, cyclin D1-CDK4/6 complex depletion, is likely to be implicated in the G0-G1 phase arrest.Generally speaking, eugenol mediated mitigation of CDK4/6 is expected to permit continuous retention of E2Fs transcription factors by the retinoblastoma tumor suppressor (RB) thus refraining cell cycle progression 47 .Besides, shortening in TFDP1 gene, a heterodimeric partner of activator E2F, will almost certainly inhibit DNA binding and activation of target genes 48 .Even though the RB family members are primarily known for inhibiting transition to the S phase, ablation of the cell cycle repressor RBL2 (Retinoblastoma-like 2) might be related to its antiapoptotic role 49,50 .This example illustrates the connection between the cell cycle and cell death 51 .www.nature.com/scientificreports/Contrary to cyclin D1, cyclin D2 upregulation by the effect of eugenol may contribute to induction and/or maintenance of a non-proliferative state, possibly through nuclear sequestration of the CDK2 catalytic subunit 52 , the expression of which was found to be downregulated.This is consistent with the outcome observed on cyclin E1 and can be explained by the fact that CDK2/E-type cyclins complex is not required due to obstruction of G1/S transition 53 .Of note, cyclin D2 is also expected to be associated with CDK4 depletion during growth arrest 52 .
On the other hand, cyclin-dependent kinase 5 regulatory subunit associated protein 1 (CDK5RAP1) inhibition by eugenol reflect maintenance of the CDK5 kinase activity.The later is known to favor apoptosis and to block the cell cycle at the level of the G0/G1 phase through direct interaction and sequestration of cyclin D1 and E2F1 in the nucleus 54,55 .Beside the phosphorylation status and the cyclin partner availability, CDK activity is further modulated by the increase in p15 INK4B , p21 CDKN1A and p27 CDKN1B56 CDK inhibitory proteins (CDKI) 57 .Furthermore, it appears that SCF SKP2 ubiquitin ligase component SKP2 downregulation in response to eugenol limited the degradation of p21 and p27 and thus loss of oncogenesis control At this level, the NUCKS1-SKP2-p21/p27 pathway is recognized as a checkpoint for G1/S transition 58 .
The modified factors also corresponded to key S phase components where eugenol is thought to restrict MCM2-7 complex formation and eventually DNA binding and replication obstruction 59 .Besides replication promotors, we noticed alterations in two major cell cycle checkpoints: The ATM/CHK2 and the ATR/CHK1 60,61 following eugenol supplementation.In fact, CHEK2 downregulation together with its downstream effectors BRCA2 62 signal a preference towards apoptosis rather than DNA repair and subsequent cell cycle progression.Furthermore, upregulation of the RAD1 component of the RAD9/RAD1/HUS1 complex doesn't seem sufficient to induce ATR-dependent CHK1 activation and repair despite the damage inflicted to the cells 63 .Cell cycle checkpoint ATM and ATR are reported to control directly several members of the MCM complex to prevent genomic damage 64 .Cyclin F CDK, reduced by eugenol, is know to be capable of initiating checkpoint response in G2 65 and to ensure mitosis fidelity through control of centrosome duplication 66 .Dual roles have been described for cyclin F 67,68 , and our results follow the example of the ovarian cancer where cyclin F enhanced proliferation and invasion of cancer cells and was linked with a poor prognosis in patients 68 .Another extensively described checkpoint process downregulated by eugenol involves the APC2 (also known as ANAPC2) catalytic subunit of the anaphase promoting complex (APC/C).APC, reigning during the anaphase to the end of the G1 phase, guarantees proper cell growth and division through modulation of multiple processes including chromosome segregation.Following the example of acute myeloid leukemia, we encourage exploring the potential of APC/C as a molecular biomarker for oral cancer prognosis 69 .
Being well documented in the literature, the possible effect of eugenol on apoptosis was explored 32 .As per our results, it appears that cell death was imposed through PARP1 modulation.In fact, protein poly(ADPribosyl)ation (PARylation) by poly(ADP-ribose) polymerase 1 (PARP1) is implicated in DNA repair among other intracellular processes.More specifically, PARP1 suppression leads to accumulation of DNA errors and sensitizes cancer cells to death in the presence of conventional anti-cancer drugs options.All of this encourages the potential use of eugenol-cisplatin combinations for the management of cancer 70,71 .On the other hand, the pro-apoptotic BCL-2 family member Noxa is strongly inhibited by the action of eugenol.Given that Noxa depletion is a common mechanism of drug resistance, better outcomes in the form of complete tumor regression and durable remission, might require overcoming Noxa destabilisation 72 .Based on the QPCR array data, death induction by eugenol is credited to multiple other proteins implicated in pyroptosis as well as in the extrinsic and intrinsic apoptotic pathways.As for the extrinsic apoptotic pathway, death receptors activation (Fas, TNFRSF10B, TNFRSF9), death ligands availability (TNF, TNFSF8) and apoptotic initiators activation (caspase 10) are the determinants of eugenol action at this level.Regarding the intrinsic mitochondrial pathway, this accounts mainly on the translational upregulation of the initiator caspase 9, DIABLO and BCL2L11/Bim 73,74 .Furthermore, an inflammatory form of apoptosis, seems to be heavily targeted by eugenol.More closely, 15.61 folds increase at the level of the inflammatory caspase 5 signal inflammasomes assembly and pyroptosis induction 75 thus enabling cell perforation as well as cytokine maturation and release 76 .Pyroptosis is known to be triggered by other chemotherapy agents and natural compounds 76 , including cisplatin 77 .Attention directed towards eugenol mediated inflammation could be of a great interest to understand drug functional characteristics.
From another angle, eugenol capacity to hinder invasion merits special attention due to promising attenuation of disease aggressivity.In our study, we were able to show that eugenol limited cancer cell migration probably due to altered matrix metalloproteinases (MMPs) secretion.More specifically, decreased MMP1 collagenase and MMP3 stromelysin levels were detected in Ca9-22 cells.At this level, a reduction in extracellular matrix (ECMs) degradation and modulation of cell behavior and cell biophysical properties relevant to invasion by means of integrins, focal adhesion kinase 78 and cell contractility modulation 79 should be considered.As for SCC-9, MMP3 upregulation and formation of MMPs complexes lacking proteolytic activity are expected to be the causal agents for tongue cancer cells migration restriction.The results at the level of MMP3 are conflicting and can be explained by the fact that this specific protease behavior is context dependent.For instance, MMP3 favors breast cancer progression while being a protective agent promoting leukocytes recruitment in skin carcinogenesis 80 .These results are particularly encouraging for exploring eugenol impact on the angiogenesis process as elastolytic MMP3 are known to generate biologically functional angiogenesis inhibitor, angiostatin 81 .On the other hand, high molecular weight MMPs complex (130, 170, and 220 kDa) formation ensure stable sequestration of MMP2, MMP9, TIMP1 (tissue inhibitors of metalloproteinases), and enzyme stabilizer NGAL (neutrophil gelatinaseassociated lipocalin) 82 .Given that the MMP complexes are detected in biological fluids, further investigation is required for their adoption as a tongue carcinoma diagnosis signature 83 .
Our last aim was to explore the cell signaling molecules carrying the message instructed by eugenol.Our results showed upregulation of the STAT5 and p38 phosphorylation levels as opposed to NF-κB.STAT5 tumor suppressor activities were previously demonstrated in breast cancer and chronic liver disease patients.This is in line with a study showing that loss of STAT5 in mouse embryonic fibroblasts and hepatocytes reduced the expression of the CDKIs p15 INK4b and p21 CIP thus leading to enhanced cell cycle progression.Other anti-oncogenes including SOCS1, p53 and PML were also shown to be activated by STAT5 in the context of differentiation and senescence regulation 84  www.nature.com/scientificreports/environmental and genotoxic stresses, might derive from its capacity to induce dormancy, promote apoptosis, block differentiation and suppress metastasis.In this respect, it should be pointed out that tumor requirements are completely stage-dependent and that more advanced tumor stages can benefit from high p38 levels 85 .Quite on the contrary, aberrant NF-κB activation is associated with multidrug resistance and is identified as a tumor signature that drives apoptosis evasion, disease recurrence and therapy resistance in both solid and haematological malignancies.In the context of the life/death balance, proliferation, migration, autophagy and necroptosis processes are also revealed to be under the influence of the NF-κB pathway 86,87 .However, considering that all the aforementioned signaling messengers can act as either malignant promotors or tumor suppressors according to the circumstances 85,88,89 , treatments should focus on balance restoration rather than complete activation or inhibition of certain signaling molecules 84 .Due to the unveiled complexity, attention is to be directed towards the eugenol natural compound.
As per the global cancer observatory, it is predicted that the incidence and mortality corresponding to oral squamous cell carcinoma will score an increase by up to 40% in 2040 90 with an estimated elevation in female patients affected 91 thereby urging more efforts at the level of disease prevention and proper management.Following the examples available in literature, our study provides a solid ground to go and assess eugenol efficacy, whether alone or in combination with chemotherapy, in animal models 35,36 and raises multiple questions regarding introduction to clinical settings.Although considered safe at a dose of 2.5 mg/kg body weight and commercially available for multiple applications such as food flavoring since 1940, clinical trials evaluating its potential for the management of oral cancer has not been launched for the moment 28 .Multiple factors should be taken into consideration before administering the eugenol drug in humans.This mainly includes the routes of administration, dose selection, drug interactions and patient population 92 .
Based on the fact that sequential administration of eugenol is proposed 35 mainly in the event of chemotherapy drug resistance 36 , repetitive intravenous administration might be overwhelming for patients.Thus, oral, and topical routes can be considered.At these levels, multiple scenarios can be adopted based on available literature data.For instance, modeling after the black raspberry mucoadhesive gel success 93 , topical application of eugenolbased paste is rather suggested for premalignant lesions management.This is attributed to limited cancer site accessibility.It is noteworthy that eugenol paste demonstrated tolerability and effectiveness in preventing alveolar osteitis as well as in supporting wound healing in 270 patients having their third molar extracted 94 .Dissolvable troches can also be an option as they ensure prolonged oral mucosa contact time.In this context, one paper reported that black raspberries administration in the form of troche allowed successful targeting oral squamous cells carcinoma tissues and reduced antiapoptotic and proinflammatory molecular biomarkers 95 .However, following oral administration of gelatin capsules containing eugenol in male and female healthy volunteers, eugenol bioavailability was questioned as it was shown to rapidly peak in blood before being metabolized and almost entirely excreted in the urine after 24 h 29,30 .Other issues to be considered are its low solubility in water, physiological barriers and targeted delivery of high drug concentrations to cancer sites.To tackle these challenges, delivery systems including liposomes, nanoparticles and phospholipid complexes can be implemented 96,97 .For instance, hydrogels containing eugenol-loaded solid lipid nanoparticles improved delivery by at least sixfold to fungi infected cells 98 .Enhancing thermal stability of inclusion complexes may also ensure slow release of eugenol 28 .Finally, customizing treatment according to patients' needs and offering precise therapies, mainly in terms of personalized dosage, is paramount to enhance therapeutic effectiveness based on the differences observed between the gingival and tongue squamous carcinoma cell lines 99 .

Conclusion
Eugenol effectiveness covers gingival carcinoma following the example of other cancer variants.Our drug was also shown to be tumor-selective, and its therapeutic potential was declared inconsistent relative to oral cancer subtypes with tongue carcinoma being more resistant.In summary, eugenol use as an adjuvant treatment option, either alone or in combination with chemotherapy, merits further investigation for the management of gingival carcinoma in patients with advanced disease state.

Figure 3 .
Figure 3.Effect of eugenol on cell apoptosis.(A) and (B) Flow cytometry data categorizing Ca9-22 cells into viable, early apoptotic, late apoptotic and necrotic based on Anx V and PI detection analysis.The cells were treated with different concentrations of eugenol for 24 h (n = 3).(C) Noxa (n = 4) and Pro-PARP1 (n = 3) protein expression due to the effect of 200 µM eugenol.The same time frame was adopted.Presented data are expressed as mean values ± SEM of three to four independent experiments.*p < 0.05, **p < 0.01, ***p < 0.001 and ****p < 0.0001 were considered as statistically significant.(D) QPCR array data corresponding to the gene expression profile of apoptotic Ca9-22.A total of 84 markers were analyzed following incubation with 200 µM eugenol for 24 h.Only the genes displaying over two-fold variation were taken into consideration (n = 1).(E) Recapitulation of pro-and anti-apoptotic markers modulated by eugenol.All markers highlighted in red were downregulated.This indicative study corresponds to only one experiment (n = 1).

Figure 4 .
Figure 4. Effect of eugenol on Ca9-22 cells migration.(A) and (B) Tracing scratch healing capacities through estimation of scratch diameter alterations following administration of different eugenol concentrations.Figures were taken at the beginning of the experiment and after 24 h.Scale bars corresponds to 500 µm (n = 4).(C) pro-MMP2, pro-MMP9 (n = 3), (D) pro-MMP1 (n = 6) and (E) pro-MMP3 (n = 6) expression as per the gelatin zymography and QPCR assays.Presented data are expressed as mean values ± SEM of three to six independent experiments.****p < 0.0001 were considered as statistically significant.

Table 1 .
Effect of eugenol on Ca9-22 expression profile of cell cycle genes.Table presenting Unigene andRefseq database identifiers all along with genes symbols and description for all cell cycle markers showing discrepancies in response to administration of 200 µM eugenol for 24 h.A total number of 84 cell cycle genes were investigated by QPCR array and only the factors exhibiting over two-fold variation were taken into consideration.This indicative study corresponds to only one experiment (n = 1).
. However, few studies have been carried out to validate its effects on oral cancer, and even less is available on gingival carcinoma, one of the common types of oral cancers.Although Teho Koh et al. failed to demonstrate the potent tumor specific effect Vol:.(1234567890) Scientific Reports | (2024) 14:10958 | https://doi.org/10.1038/s41598-024-60754-8